联系电话:13162931356
固定电话:0571-89925175
公司地址:杭州市西湖区金蓬街366号2号楼506,512室
MarkerGeneTM Glucuronidase (GUS) Reporter GeneActivity Detection Kit
背景描述:
报告基因普遍用做“标志物 Markers”对基因调控和定位分析,以及突变基因分析。通过免疫实验,生化活性或组织化学分析来对组织或细胞的报告基因表达进行检测。
大肠杆菌来源的β-葡萄糖苷酶(β-glucuronidase,GUS)普遍认为是转基因植物研究中非常理想的报告基因(marker gene)。GUS报告基因系统具有许多优势,包括稳定表达大肠杆菌GUS,不会干扰正常植物代谢和高等植物内几乎无内源性GUS活性。
数种葡萄糖醛酸底物可用来检测GUS表达,这些底物都包含糖基D-葡萄糖醛酸苷(D-glucopyranosiduronic acid)通过糖苷键连接到生色底物、荧光底物或其他检测分子的—OH。体外用于GUS活性检测的最广泛使用的荧光底物为MUG(4-Methylumbelliferyl beta-D-glucuronide,4-甲基伞型酮-beta-D-葡糖苷酸,CAS:6160-80-1或881005-91-0)。一旦被水解,生成荧光素4-MU(4-甲基伞型酮)和β-D-葡萄糖醛酸。
检测原理:
本MarkerGeneTM GUS报告基因活性检测试剂盒(MarkerGeneTM Glucuronidase(GUS) Reporter Gene Activity Detection Kit)以MUG为荧光显色底物。当植物或其他细胞用GUS萃取液(含磷酸-EDTA,pH 7.0和去污剂)萃取后,所得到的萃取液(含GUS)能水解4-MUG生成4-MU(4-甲基伞型酮,pKa 8.2)和β-D-葡萄糖醛酸。加入碳酸钠缓冲液终止该反应(因4-MU在pH值高于pKa的情况下发射最大荧光信号)。4-MU的最大激发波长为365nm,最大发射波长为455nm。
试剂盒组分:
|
组分名称 |
组分编号 |
规格 |
保存 |
|
GUS Extraction Buffer |
0877-001 |
25 mL |
Store cold (4℃) |
|
Carbonate Stop Buffer |
0877-002 |
25 mL |
Store cold (4℃) |
|
GUS Assay Buffer |
0877-003 |
5 mL |
Store cold (4℃) |
|
4-MU calibration stock solution |
0877-004 |
5 mL |
Store cold (4℃) |
订购信息:
|
货号 |
产品名称 |
规格 |
价格(元) |
|
M0877 |
MarkerGene™ β-Glucuronidase (GUS) Reporter Gene Activity Detection Kit |
1Kit |
5680.00 |
使用文献(MarkerGene™ β-Glucuronidase(GUS) Reporter Gene Activity Detection Kit):
Hesari N, Alum A, Elzein M, Abbaszadegan M. (2016) "Abiosensor platform for rapid detection of E. coli in drinking water."Enzyme and Microbiol Tech 83: 22-28.http://dx.doi.org/10.1016/j.enzmictec.2015.11.007
Almeyda CV, Raikhy G, Pappu HR. (2015) "Characterization andcomparative analysis of promoters from three plant pararetroviruses associatedwith Dahlia (Dahlia variabilis)." Virus Genes. 51(1):96-104
Li L, Song Y, Wang K, Dong P, Zhang X, Li F, Li Z, Ren M. (2015)"TOR-inhibitor insensitive-1 (TRIN1) regulates cotyledons greening inArabidopsis." Front Plant Sci. 6:861.
Shepherd DN, Dugdale B, Martin DP, Varsani A, Lakay FM,Bezuidenhout ME, Monjane AL, Thomson JA, Dale J, Rybicki EP (2014)"Inducible Resistance to Maize Streak Virus." Lin B, ed. PLoS ONE9(8):e105932. doi:10.1371/journal.pone.0105932.
Chen Y, Yordanov YS, Ma C, Strauss S, Busov VB. (2013) "DR5as a reporter system to study auxin response in Populus." Plant Cell Rep.32(3):453-63.
Behringer C, Bartsch K, Schaller A. (2011) "Safeners recruitmultiple signalling pathways for the orchestrated induction of the cellularxenobiotic detoxification machinery in Arabidopsis." Plant Cell Environ. 34(11):1970-85.
Horváth BM, Magyar Z, Zhang Y, Hamburger AW, Bakó L, Visser RG,Bachem CW, Bögre L.(2006) "EBP1 regulates organ size through cell growthand proliferation in plants." EMBO J.25(20):4909-20.
